CA2174628C - Novel spin trap nitronyl hindered phenols - Google Patents

Novel spin trap nitronyl hindered phenols Download PDF

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Publication number
CA2174628C
CA2174628C CA002174628A CA2174628A CA2174628C CA 2174628 C CA2174628 C CA 2174628C CA 002174628 A CA002174628 A CA 002174628A CA 2174628 A CA2174628 A CA 2174628A CA 2174628 C CA2174628 C CA 2174628C
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compound
tert
alkyl
butyl
nitronyl
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CA2174628A1 (en
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Edward G. Janzen
Allan L. Wilcox
Randall D. Hinton
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Oklahoma Medical Research Foundation
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Oklahoma Medical Research Foundation
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Abstract

The invention is the use of nitronyl substituted hindered phenols as antioxidants in therapeutic applications. In the preferred embodiment the compositions have general formula (I), wherein R1 is hydrogen, an alkyl or an aryl and R2 is an alkyl or an aryl; R3 is an alkyl; and R4 is an alkyl.
Further, the invention relates to novel compositions useful as antioxidants.
The novel compounds include: 2,6-di-<u>tert</u>-butyl-4-(N-<u>tert</u>-octyl) nitronyl phenol (DBONP); 2,6-dimethyl-4-(N-<u>tert</u>-octyl) nitronyl phenol (DMONP); N-<u>tert</u>-octyl-C-phenyl nitrone (OPN).

Description

NOVEL SPIN TRAP NITRONYL HINDERED PHENOLS
TECHNICAL FIELD OF THE INVENTION
The present invention relates to novel nitronyl substituted phenols. The present invention also relates to methods using nitronyl substituted hindered phenols as antioxidants in biological systems and therapeutic applications.
a .a . i._. .

~'-34966PCT
.- ~ ~~- ~ ~~1~~628 .
BACKGROUND 'OF THE~INVENTION .
The use of antioxidants has been proposed for therapeutic treatment and for other uses such as protecting polymers.such as natural rubber and synthetic .
rubber from oxidation. Hindered phenols occur naturally, for example tocopherols (vitamin E), and have found use as antioxidants previously. Recently, free radicals have been postulated to-have significant impact in tissue injury. Evidence. suggests that the free radical mechanism has a significant impact on vascular injury and damage affecting nerve cells.
The use of phenylbutyl nitrone compositions for the treatment of oxidative tissue damage and gastric ulceration has been disclosed in U.S. Patent No.
5,025,032 entitled "Phenylbutyl Nitrone Compositions and Methods For Treatment of Oxidative Tissue Damage," U.S.
Patent No. 5,036,097 entitled "Phenylbutyl Nitrone Compositions and Methods for Prevention of Gastric Ulceration," and International Application Serial No.
PCT/US92/05T94 (Publication No. W092/22290) entitled "Use of Spin Trapping for the Treatment of D~:seases Associated with Oxidation of Lipids and Proteins."
Research~has demonstrated that nitrones select a location in membrane models and microsomes which is as polar and/or as protic as pure methanol as discussed in D.L. Haire et al., "Locating spin traps in heterogeneous media by 13C NMR. Investigations in SDS micelles DMPC
vesicles and rat liver~microsomes", J. Org. Chem.
54:2925-2920 (1989). Thus, it is suggested that w -30 antioxidant molecules must be precisely located in the same volume compartment as where the free radical event occurs, or else the free radicals will not be quenched.
Heretofore, such molecules have not been available.
Therefore, development of new families of antioxidant RMENDED SHEET

~-34966PCT
. '~'"'.
molecules is necessary in order to provide molecules which will be effective against free radical damage at different biological sites. There has also been a need to .provide antioxidant compositions which have no known toxic effect while providing a more effective free radical spin trap.
The present invention offers the advantages of a spin trap agent with no known toxic effects. Further, the invention offers the advantage of. providing compounds highly efficient in the quenching of free radicals.

;~ -34966PCT
SOI~iARY OF THE INVENTION
. The present invention relates to the use of particular antioxidants in therapeutic treatment. These compositions have the following general formula:
~R1 HO ~ ~ C\
N+ R2 R3 . O-wherein R1 is a hydrogen, an aryl, or an alkyl and R2 is an alkyl or an aryl group. Rl can be any alkyl group, straight chain or branched, with or Without double or .
triple bonds, with or without polar functions (e. g., esters, alcohols; halides, carboxylic acid, aldehydes, carboxamides, aralkyl, amino or nucleic acids). R2 can contain single, double or triple bonds and may also include polar constituents (e. g., esters, alcohols, halides, carboxylic acids, aldehydes, carboxamides, aralkyl, amino or nucleic acids). R2_can also be an aryl including substituted aryls, heterocyclic, polycyclic or acyclic. R3 and R4 can be hydrogen or any alkyl group, either straight chain or branched, preferably having l to 4 carbons atoms. R3 and R4 are preferably~alkyls having l:to 4 carbon atoms. R3 and R4 are usually the same group. Based on animal studies the dosage of these compounds is in the range of 25 to 250 mg/kg. In the preferred embodiment, the range is between 25 and 12.5 mg/kg depending upon the dosage required to capture the free radical. One or more of the above compounds useful in the present invention can be mixed together in the same dose.

~1'~4~2~
The present invention also.relates to the use of compounds of a general formula:
C'H CH3 ~ CH3 ~N+ C-CH2-C-CH3 CH3 CH3.
Based upon animal studies, the dosage in the range of 25 to 250 mg/kg is useful. In the preferred embodiment; the 5 range is between 25 to 125 mg/kg.
The present invention also relates to the use of compounds of the general formula:

H ~ ~ C' ~N+ R5 R6 R9 O_ wherein R5, R6, R7, RS and R9 are alkyl groups, and preferably R5, R6, R7, R8 and R9 are alkyls having 1 to 4 ~ carbon atoms. It is believed that these compounds would be useful in a dosage range of from 25 mg to 250 mg/kg of body wefight.
Another aspect of the present invention relates t,o novel compounds of the formulas useful as spin traps in biological systems:

WO 95/11227 ~ PCT/US94/12107 (a) N-tert-octyl C-phenyl nitrone ("OPN") C'H CHg CH3 ~N+ C-CH2-C-CHS ' CHg CH3 (b) 2,6-di-tert-butyl-4-(N-tert-octyl) nitronyl phenol ("DBONP") CHg H3C-C-CHg H
' CHg CH3 ~ + CH3 CH3 CHg (c) 2,6-dimethyl-4-(N-tert-octyl) nitronyl phenol ("DMONP") H ~ ~ C'H CHg CH3 ~N+ C-CH2-C-CH3 H3C O- CHg CH3 and (d) compounds of the general formula ~, ~~~t ~ _, ~ w ' ~, .,.,~'~:, r ~.,i~., ~~"-. , '~-34966PCT
. , ~ . 2~'~4~2~
~ ~ ,H
c ~~
~N+-Ri p ~_ wherein Rlo is an alkyl having 9 or. more carbon atoms.
Such compounds are to be used in the method of the present invention in a dosage from 25 to 250 mg/kg, preferably-from 25 to 125 mg/kg, and more preferably from 25 to 50 mg/kg.
~~.'~~628 BRIEF DESCRIPTION OF THE DRAWINGS
The invention will be more fully appreciated from the following description taken in conjunction with the ' accompanying drawings, in which:
FIGURE 1 is a graphical representation of inhibitor ' concentration for 50% inhibition (ICso) using rat liver microsomes (RLM) wherein LPO (liquid peroxidation) was initiated by tert butoxyl radicals and MDA
(malondialdehyde) production was monitored by treatment with thiobarbituric acid;
FIGURE 2 is a graphical representation of inhibitor concentration for 50% inhibition (ICSO) using rat liver microsomes where LPO is initiated by NADPH catalyzed cytochrome - P450 metabolism of CC14 based on the TBA
(thiobarbituric acid) test for MDA production; and FIGURE 3 is a graphical representation of inhibitor concentration for 50% inhibition (ICso) of LPO for rat brain microsomes (RBM) using the TBA test for MDA
production.
-r.
_ . ,~ ~. , ~ ; _, ~'jn;.'~
DETAILED DESCRIPTION OF THE INVENTION
As used herein a free radical scavenger or spin trap reagent (compound) is a molecule which will form a stable complex with a free radical. A carbon centered free radical is a molecule in which the free radical is localized on a carbon atom. As result of this chemical bond formation with a spin trap, the free radical is no longer damaging to cells.
Antioxidant activity has been long studied in lubricating oils by the automobile industry. The general principles and mechanisms from the lubricating oil studies has been accepted for lipid peroxidation in tissue membranes. In addition, without being bound to any particular theory we believe that there are some specific considerations which are specific to biological systems. Reactive radicals which can be damaging to tissue constituents are easily quenched by the phenolic hydrogen which is easily removed by most free radicals.
X ~ + H ~ ~ Y ---~ ~ O ~-~ Y
Any Phenol Phenoxyl reactive radical radical This reaction produces non-damaging radicals, that is radicals that are resonance stabilized and have little reactivity. The phenoxyl radicals, in general, have been observed to disappear without creating obvious biological damage.
It has been found in biological systems that phenoxyl radicals which are stabilized by steric ~1'~462~

hinderance due to groups at the 2-and 6-position have an added advantage that they persist: long enough to trap other radicals thereby quenic~ing two radicals. For ' example, it has been found that 2,6-di-tert-butyl phenols 5 produce 2,6-di-tert-butyl phenoxyl radicals which are stabilized due to the steric hinderance of the tert-butyl groups. The hindered phenoxyl has the advantage that they persist long enough to trap other radicals.
CH3 CHg CH3 H3C-C-CH3 H3C-C-CHg H3C-C-CH3 H ~ ~ Y ~ .O ~ ~ Y X~ O Y
X
H3C-C-CHg H3C-C-CH3 H3C-C-CH3 To increase the efficiency of the antioxidant 10 activity and achieve maximum potential, it is desirable to utilize a compound which produces a high concentration of the hindered phenoxyl which will be available to capture the additional free radicals. .
It is preferred that the compounds used in the present application have a reasonably long lifetime to increase efficiency. The rate of the first reaction depends upon the concentration of phenol and free radical. The rate of the first reaction is the first reaction rate constant times the concentration of the phenol times the concentration of free radicals. The rate of the second reaction depends on the concentration of the hindered phenoxyl and concentration of free , radical. The reaction rate of the second reaction is the I,,' WO 95/11227 PCT/US94/12107 ~~'~4628 1~
value of the second reaction rate constant, times the concentration of phenoxyl times the concentration of free radical. Thus, it is beneficial to use compounds which result in maximum concentration of phenoxyl.
The appropriate choice of the substituent in the 4-position (Y) can increase the lifetime of the hindered phenoxyl radical produced. The groups in the 4-position which stabilize the hindered phenoxyl radicals also reduce the reaction rate of the radical with oxygen thereby preventing formation of potentially damaging peroxyl radicals. For example:
CHg CH3 CH3 H3C-C-CHg H3C-C-CH3 H3C-C-CH3 O ~ ~ Y ~ Y +p2 ~- O
Op H3C-C-CHg HgC-C-CHg H3C-C-CH3 The reaction with oxygen at the 4-position can be hindered by several methods. For example, steric hinderance may be utilized, and generally, the reaction is slowed but not entirely eliminated.

WO 95/11227 PCT/US94/12107 , J;
~~ ~4 ~2~

CH3 CHg HgC -CHg H3C-C-CH3 CHg 3 _ ~--~ C-CH3 + 02 ~ O CI H CHg CHg ~ 3 CHg CHg Another method is to provide resonance with the carbon in the 4-position. When the ethylenic bond is obtained, a completely stable phenoxyl radical is obtained. Thus, groups capable of strong resonance with the phenoxyl function stabilize the phenoxyl radical and prevent an addition reaction with oxygen.

O ~ r--C°C ~o ~-.
H3C-C-CHg ~~'~4~2$

Another method of stabilization is the addition of a strained ring or rings-within the phenoxyl radical adduct.
Thus, when Y is a phenoxyl ring such as a-tocophenoxyl addition of oxygen is not favored. It is believed that the strained bicyclic ring structure in the peroxyl radical is a high energy product, and the formation of the peroxyl from oxygen is very unfavorable.
CH3 CHg CH3 ~ O O
\ \
\ ~ I'CHg E--r CH3 + 02 CH3 HgC ~ ~O~CH3 HgC \ O CH H C \ O CH
CHg CH3 3 3 H3C O\O 3 These phenoxyl radicals with strained rings can be beneficial because although they will not readily react with oxygen radicals, reactions may proceed with other peroxyl radicals to form stable adducts.
Compounds which are useful in the present invention have the following general formula:
,R1 ~N+ R2 )_ where R1 is hydrogen, an aryl, or an alkyl and R2 is an alkyl or an aryl. The alkyls of R1 and R2 can contain single, double or triple bonds and can also include polar ~ ~..# °..''.. ?'1' constituents like esters, alcohol; halides, carboxylic acids, aldehydes, carboxamides, aralkyl amino or nucleic acids and others. R1 and R2 can also be an aryl including substituted aryls, heterocyclic, polycyclic or acyclic.
R3 and R4 can be any alkyl group, either straight chained or branched. Preferably, R3 and R4 are alkyls having 1 to 4 carbon atoms. In the preferred embodiment, R3 and R4 are the same group because synthesis of such compounds is . typically easier than when R3 and R4 are different.
Other compounds useful in the present invention and which are novel,compounds have the general formula:
/ ~ 'H
C
~t~RlO
~_ wherein Rlo is an alkyl having 9 or more carbon atcms.
Preferably, 2,6-di-tert-butyl-4-(N-tert-butyl) nitronyl phenol (DBBNP):

H3C-C-CH3 . .

H ~ ~ C'H
N+ C-CH3 H C- ~ C CH3 3 . 3 ~1'~46~~
or 2,6-di-tert-butyl-4-(N-tert-octyl) nitronyl phenol (DBONP) H3C-C-CHg H ~ ~ C'H

w N+ C-CH2-C-CH3 H3C-C-CH3 ~ CH3 CHg are employed in a method for quenching biological free radicals. Less preferred compounds for said method 5 include 2,6-dimethyl-4-(N-tert-octyl) nitronyl phenol ( DMONP ) HgC
H
H ~ ~ C\ CHg CH3 H3C ~' + CH3 CH3 and 2,6-dimethyl-4-(N-tert-butyl) nitronyl phenol (DMBNP):

'H CH
H C ~ 3 N+ C-CHg H3C ~' CH3 Another novel compound useful in the present invention is N-tert-octyl C-phenyl nitrone (OPN) which is represented below.
C'H CH3 CH3 ~N+ C-CH2-C-CHg Spin traps have been implicated as useful in a number of diseases including septic shock, effect of ischemia/
reperfusion, liver edema, and fatigue stress. The spin trapping efficiency is believed to be associated with not only the molecular configuration but also the relative size of the molecule in respect to the particular disease sought to be prevented or treated. Thus, certain spin trap compounds may be more effective with certain diseases than other spin trap compounds.
Spin trap compounds of the present invention were placed in pharmaceutical vehicles suitable for administration to a patient, preferably in a fat soluble ~~'~~~~$
m substance for oral administration. The spin trap compounds of the present invention are useful in preventing or reversing edema. The compositions can also contain other active agents, such as buffering agents such as antacids or inert carriers such as lactose.
The examples demonstrate the utility of the compounds of the present, invention in preventing or treating a variety of inflammation effects. Exemplary doses range from 25 to 250-mg of compound/kg of body weight in animals. The more preferred range of dosage is from 25 to 125 mg/kg. The effective range of dosage in humans and other mammals is expected to be between 25 to 50 mg/kg, and preferably between 25 to 35 mg/kg of body weight. The particular,dosage may vary depending on the particular compound selected and the disease to be treated. Those compounds which are more effective will require a smaller dosage than those compounds which have been found to be less effective. For preferred embodiments of the invention; the°effective range of dosage in humans and other mammals is expected to be in the range of: (a) from to 50 mg/kg for DBBNP; (b) from 25 to 50 mg/kg body weight for DBOMP; (c) from 25 to 50 mg/kg.of body weight for DMONP; (d) from 25 to 50 mg/kg of body weight for DMPNP; and (e) from 25 to 50 mg/kg of body weight for OPN.
25 The most preferred ranges are expected to be (a) from 25 to 35 mg/kg for DBBNP; (b) from 25 to 35 mg%kg body weight for DBOMP; (c) from 25 to 35 mg/kg of body weight for DMONP; (d) from 25 to 35 mg/kg of body weight for DMPNP;
and (e) from 25 to 35 mg/kg of body weight for OPN.
~ Other compounds believed to be useful include °
compounds of the general formula:

'~-34966PCT
~1'~ 46~~
la R7 ~
w R6 R9 O.
wherein R5, R6, R7, R8 and R9 are alkyl groups, and preferably alkyl groups having 1. to 4 carbon atoms. These compounds are expected to~be useful in dosages from 25 to 250 mg/kg of~body weight, preferably 25 to 125 mg/kg and more preferably from 25 to 50,mg/kg of body weight.
The compounds of the present invention are preferably administered. systemically, most preferably orally,_.since this is the most rapid and efficient means for delivering the active compound to the site of free radical .
generation. The compounds can be administered at once, or can be divided into a number of smaller doses to be administered at varying intervals of times. The compounds may also be administered by other methods including intravenous, subcutaneous, topical, and intraperitoneal administration.
A preferred. method of administration of the compounds of the present invention is oral delivery. The compounds may be'enclosed in capsules, compressed into tablets, microencapsulated, entrapped in liposomes, in solution or suspension, alone or, in combination with.a substrate immobilizing material such as starch or poorly absorbable salts. Pharmaceutically compatible binding agents and/or adjuvant materials can be used as part of a composition.

~~,~ 4~~g Tablets or capsules can contain any of the following ingredients, or compounds of similar nature: a binder such as microcrystalline cellulose, gum tragacanth or gelatin;
an excipient such as starch or lactose; an integrating ' S agent such as alginic acid, Crimogel°, or corn starch; a lubricant such as magnesium stearate or Sterotes; a glidant such as colloidal silicon dioxide; and sweetening and flavoring agents. When a capsule form is used the liquid carrier such as a fatty oil may be used. Capsules and tablets can be coated with sugar, shellac and other enteric agents as is known.
The present invention will be further understood by reference to the following nonlimiting examples demonstrating methods for determining the effectiveness of the compounds of the present invention for the treatment or prevention of inflammation effects, septic shock, effects of ischemia/reperfusion, liver edema, fatigue stress.
Compounds useful in the method present of the present invention were compared against (a) butylated hydroxy toulene ("BHT") H3C~C OH C~CH3 H3C \ CH3 CHg I f!

(b) a-phenyl t-butyl nitrone ("PBN") ~H
C\ CH3 N+ C-CHg ~- CH3 and (c) a-tocopherol (Vitamin E) .
Inhibition of lipid peroxidation of rat liver microsomes has been found to be remarkably effective 5 utilizing 4-nitronyl hindered phenols. The efficiency of these compounds was compared to the inhibition characteristics of a hindered phenol antioxidant, butylated hydroxy toluene (BHT) and a-phenyl t-butyl nitrone (PBN). Comparisons were also made with compounds 10 useful in the present invention as well as the novel compounds of the present invention 2,6-di-tert-butyl-4-(N-tert-octyl) nitronyl phenol (DBONP); 2,6-dimethyl-4-(N-tert-octyl) nitronyl phenol (DMONP); and N-tert-octyl-C-phenyl nitrone (OPN).
15 EPR samples from the in vivo experiments were run on a Bruker 30OE Electron Paramagnetic Resonance Spectrophotometer. Two milliliters of sample were placed in a quartz tube of 2 mm inside diameter. EPR parameters were as follows with the exception of the receiver gain 20 and scale. These are adjusted for each sample to get the best signal.

i.
_~ ~.

Receiver Signal Channel Receiver Gain l.OOe+05 Conversion 327.68 ms Phase 0 deg Time Const 1310.72 ms Harmonic 1 Sweep Time 335.544 ms Mod Frequency 100.0000 kHz Scale 18 Field Microwave Center Field 3480.01 G Frequency 9.77 GHz Sweep Width 100.00 G Power 1.99 a+O1 Resolution 1024 points mW
Example 1 Livid peroxidation (LPO) initiated by tert-butoxyl radicals Male Sprague-Dawley rats (175-200g) that had been maintained on commercial rat chow were starved for 24 hours, sacrificed and the livers removed. Microsomes were prepared by homogenizing the minced livers in 0.15M
potassium phosphate buffer pH 7.4 5 ml/g) and then centrifuging at 12,000 X g for 15 minutes. The supernatant fraction was then centrifuged at 105,000 x g for 90 minutes. The microsomal pellets were washed twice by resuspending in buffer and centrifuging at 105,000 x g for 60 minutes. The microsomal pellets were kept frozen at -80°C until ready for use. Rat liver microsome pellets are made up into microsomal suspension (MS) by adding one milliliter of 50mM potassium phosphate buffer (pH 7.4) per gram of liver. The protein concentration of microsomal suspensions were determined by the method of O.H. Lowry et al., J. Biol. Chem. 193:265-75 (1951).
Reaction samples were 1 ml (milliliter) in volume and consisted of MS (0.1 ml), 50 mM potassium phosphate buffer (KH2PO4 and KZH) (pH 7.4), inhibitor in alcohol (isopropyl) and initiator (DBPO) in isopropyl alcohol.

The order of addition of reagents was buffer, MS, inhibitor and finally initiator. For those experiments where the NADPH generating system is used as initiator, the reaction components were: buffer (as above), 1mM EDTA, MS, CC14 (100 mM) and generating system. The generating system consisted of 0.5 Kornberg units of glucose-6-phosphate dehydrogenase, 5~.M glucose-6-phosphate andØ3 mM NADPH. After all reagents were added, the test tubes were vortexed and placed in a 37°C shaking water bath.
Samples were incubated for one hour. A. Ottolengi, Arch.
Biochem. Biophs. 79:355 (1959). The lipid peroxidation (LPO) reaction was stopped by the addition of 0.5 ml 35%
TCA (trichloroacetic acid) (weight/volume in distilled H20) and 1.0 ml 0.5% TBA (thiobarbituric acid) (w/v in distilled Hz0). Samples were capped with glass marbles and placed in a boiling (100°C) water bath for 15 minutes, then cooled rapidly in an ice bath. One milliliter of distilled Hz0 and 2 ml chloroform were added, samples vortexed and then centrifuged at 1500 rpm for 10 minutes.
The aqueous layer was read at 532 nm on a Perkin-Elmer Lambda W/VIS spectrophotometer using a distilled Hz0 blank. MDA (malondialdehyde) calculations were made by the following equation:
(O.D. at532nmx22.4) -' mgprotein/m1 MS1- rlmolesMDAproduced 0 .1 ml MS ' mgmicrosomal protein Inhibition studies were performed by doing a concentration course of the inhibitor added to the LPO
system. A stock solution of the inhibitor was made up so that various dilutions would give several (usually five) final concentrations. The original concentrated stock was usually 1 M (molar) and dilutions were made to give the following final concentrations: 10, 1, O.l, and 0.01 mM.
Control samples had no inhibitor. Five samples were done for each concentration. After MDA values were calculated, percent of inhibition was determined by: average of MDA
values for a given concentration divided by average of MDA
values for control multiplied by 100. These results then determined if further dilutions were necessary to achieve a 50% inhibition of LPO.
Inhibitor Concentration of 50o Inhibition (ICSO) (average of 5 experiments) BHT 5.3 ~M (interpolated between 5 and 6 ~.M) PBN 9800 ~,M (interpolated between 5 and 10 mM) DBBNP 4.3 ~M (interpolated between 2.5 and 5 ~.M) DBONP 5.8 ~,M (interpolated between 5 and 7.5 ~.M) DMONP 16.4 ~M (interpolated between 15 and 20 ~M) DMBNP 230 ~M (estimated from 250 ~,M experiment) OPN 462 ~.M (estimated from 250 and 500 ~.M) Tocopherol (vitamin E) 30 ~.M (measured) In this example and the following examples, ICso was attempted to be reached by trial and error. In the event it was missed, the ICso value was determined by interpolation of the results. Interpolations were made using the closest result higher than ICso and the closest result lower than ICso. The reference to "measured" means that ICso was hit right on and thus no interpolation was required.
The test results demonstrate that the flanking tert-butyl groups in the ortho positions (2, 6) of the phenol give improved efficiency. The relative efficiency of the various compounds from the above data normalized to 1.0 for PBN can be represented as follows:

DBBNP> BHT> DBONP> DMONP> Vit E> DMBNP> OPN> PBN
2466 2000 1828 646 354 46 24 1.0 Thus, DBBNP is about 2000 times more effective as an inhibitor of LPO in rat liver microsomes than PBN and about 20% better than BHT. Even taking into account experimental precision, one can conclude that DBBNP is at least as good as BHT and probably better.
Example #2 LPO initiated by NADPH catalyzed cytochrome -P450 metabolism of CC1 An amount equal to 0.09 mmole spin trap is weighed into a test-tube to give a final concentration of 30 mM.
To this container is added 14 ~1 13CCL4 (to produce a final concentration of 50 mM). After shaking to dissolve the spin trap, 2.35 ml of 50 mM potassium phosphate buffer at pH 7.4 (KH2P04 and KzHP04) is added plus 0.3 ml microsomal suspension. The solution is vortexed and preincubated for 10 minutes at room temperature (25°C). At this point, 0.3 ml NADPH generating system (0.5 Kornberg units of glucose-6-phosphate dehydrogenase, 5 ~,M glucose-6-phosphate and 0.3 mM NADPH) is added to start the reaction. After incubation for 15 min at room temperature, 1.0 ml toluene is added and the system vortexed. Following centrifugation for 30 minutes at 3000 rpm (Sorvell GLC-4 with swinging bucket rotor H1000) approximately 500 ~,1 supernatant solution is removed and transferred to an EPR
quartz tube. The solution is degassed for 10 minutes with argon and scanned by EPR spectrometry.

The following results were obtained:
Inhibi for Concentration of 50 o Inhibi Lion (ICso) (average of 5 experiments) BHT 55 ~,M (interpolated between 50 and 100 ~.M) ' 5 PBN 17,500 ~.M (interpolated between 10 and 25 mM) DBBNP 53 ~.M (interpolated between 50 and 100 ~,M) DBONP 35 ~.M (interpolated between 20 and 40 ~,M) DMBNP 710 ~,M (interpolated between 500 and 750 ~M) DMONP 60 ~M (interpolated between 40 and 80 ~,M) 10 OPN 6500 ~.M (interpolated between 4 and 8 mM) Example #3 Rat Brain Microsomes Similar tests were performed with rat brain microsomes using the TBA test for MDA production as the result of LPO. Results on the same compounds were as 15 follows:
Inhibi for Concentration for 50 o Inhibi Lion (ICso) BHT (not available) PBN 10 0 0 ~.r.M
DBBNP 0.7 ~.M
20 DBONP 0.3 ~M
DMONP 7 0 ~,M
DMBNP 6 0 0 ~.M
OPN 76 ~.M
Although BHT was not available for this test it is not 25 believed that it would be particularly effective with this particular system.
The data obtained demonstrates that DBBNP and DBONP
are very good inhibitors in these systems.
ICso RLM ( I ) RLM ( I I ) RBM ( I I I ) 3 0 DBBNP 4 . 3 ACM 5 3 ~.M 0 . 7 ~.M ( 7 0 0 nM ) DBONP 5 . 8 ~M 3 5 ~.M 0 . 3 ~ ( 3 0 0 nM ) WO 95/11227 " PCT/US94/12107 The above data in Examples 1, 2 and 3 are graphically represented, respectively, in FIGURES 1, 2 and 3. It should be noted that in these graphs the smaller result is better.
FIGURE 1 is a graphical representation of inhibitor ' concentration for 50% inhibition (ICso) using rat liver microsomes wherein LPO (liquid peroxidation) was initiated by tert-butoxyl radicals and MDA (malondialdehyde) production was monitored by treatment with thiobarbituric acid (TBA). The relative effectiveness between the compounds can be seen, with the smaller bars indicating better performance.
FIGURE 2 is a graphical representation of inhibitor concentration for 50% inhibition (ICSO) using rat liver microsomes where LPO is initiated by NADPH catalyzed cytochrome-P450 metabolism of CC14 based on the TBA
(thiobarbituric acid) test for MDA production.
FIGURE 3 is a graphical representation of inhibitor concentration for 50% inhibition (ICso) of LPO for rat brain microsomes using the TBA test for MDA production.
SYNTHESIS OF NOVEL COMPOUNDS
Synthesis of the novel compounds of the present invention were carried out following the general procedures below.
2-Methyl-2-nitropropane was prepared as follows:
potassium permanganate (650 g, 4.1 mole) was dissolved in 3 L H20 and t-butyl amine (100 g, 1.4 mole) added over 30 minutes. The temperature was brought to 90°C and the reaction allowed to cool for 4 hours with stirring by mechanical stirrer. A still head and condensor was attached to a side arm of the 5 L three neck round bottom flask and the product distilled off. Diethyl ether was added and the product washed 2x with 5% HC1, lx with H20, lx with saturated NaCl. The organic layer was dried over MgS04 and the solvent stripped leaving 112.6g (1.09 mole, 78%) clear liquid.
4-Nitro-2,2,4-trimethylpentane was prepared as follows: potassium permanganate (380 g, 2.4 mole) was added in portions to t-octyl amine (50 g, 0.4 mole) and MgS04 x 7H20 (60 g) in 250 mL H20 with mechanical stirring.
The temperature was maintained below 30°C with an ice bath. Stirring and cooling was continued for 2.5 hours after which the reaction was allowed to warm to room temperature and stirred for 48 hours. The reaction was filtered and the residue washed with pentane. The organic layer was separated, dried over MgS04 and pentane distilled at atmospheric pressure. The product was distilled at <1 mm to give 30 g (47%) of clear liquid.
t-Octyl hydroxylamine was prepared as follows: 4-nitro-2,2,4-trimethylpentane (10.35 g, 0.065 mole) with NHQC1 (3.49 g, 0.065 mole) was cooled in 75% THF/H20 with stirring by a magnetic stir bar to l0°C and zinc (25.5 g, 0.39 mole) added in portions to maintain the temperature at 10-15°C (one hour). Reaction was allowed to warm to room temperature and stirred for one hour. The mixture was filtered and the solvent stripped leaving 9.25 g (98%) clear liquid. The hydroxyl amine was used immediately in subsequent reactions.
Example 4:
Procedure for the synthesis of 2,6-dimethyl-4-(N
tert-octyl) nitronyl phenol (DMONP) is similar to other 4-nitronylphenols. t-Octyl hydroxylamine (4.35 g, 0.03 mole) and 3,5-dimethyl-4-hydroxybenzaldehyde (2.25 g, 0.015 mole) were refluxed in 60 mL benzene with 5 mg p-TsOH for 15 hours. TLC on silica gel (20% EtOAc/hexane) showed 1:1 aldehyde (rf=0.47) to nitrone (rf=0.29).

t-Octyl hydroxylamine (4.35 g, 0.03 mole) was added and the reaction stirred for 18 hours. TLC showed no aldehyde, mostly nitrone, and a few less polar impurities.
The solvent was stripped, the residue applied to a silica gel column, and product eluted with mixtures of hexane/EtOAc to give 3.74 g (90%) crystals with a melting point of 113°-114°C.
Example 5:
2,6-di-tert-butyl-4-(N-tert-octyl) nitronyl phenol (DBONP) can be prepared as follows. t-Octyl hydroylamine and 3,5-di-tert-butyl-4-hydroxybenzaldehyde are refluxed in benzene with p-TsOH for sufficient time to begin the reaction. t-Octyl hydroylamine can then be added and the reaction stirred until complete reaction has occurred.
The solvent is then stripped, the residue applied to a silica gel column, and product eluted with mixtures of hexane/EtOAc which should produce DBONP crystals with a melting point of 153°-154°C.
Example 6:
N-tert-octyl C-phenyl nitrone (OPN) can be prepared as follows: t-octyl hydroxylamine and 4-hydroxybenzaldehyde should be refluxed in benzene with p-TsOH for sufficient time to begin the reaction.
Additional t-octyl hydroxylamine can be added and the reactants stirred until completion of the reaction. The solvent can then be stripped, the residue applied to silica gel column and product eluted with mixture of hexane/EtOAc which should give OPN crystals.
While the invention has been described by several specific examples, it will be understood that the invention is not limited to the specific examples herein.

Claims (21)

CLAIMS:
1. A compound having the formula:

wherein R1 is a hydrogen, an aryl, or a straight chain or branched alkyl with or without a polar constituent;
R2 is a straight chain or branched alkyl with or without a polar constituent, or an aryl;
R3 is an alkyl having from 1 to 4 carbon atoms; and R4 is an alkyl having 1 to 4 carbon atoms; provided that when R2 is tert-butyl R1 is not H, except in the case where R3 and R4 are both tert-butyl or methyl groups respectively, for use in the in vivo treatment or prevention of lipid peroxidation.
2. The compound of Claim 1 wherein R1 is hydrogen and R2 is an alkyl.
3. The compound of Claim 1 wherein R1 is an alkyl.
4. The compound of Claim 1 wherein R1 is an alkyl comprising polar constituents selected from the group consisting of esters, alcohols, halides, carboxylic acids, aldehydes, carboxamides, aralkyl, amino and nucleic acids.
5. The compound of Claim 1 wherein R2 is an alkyl comprising polar constituents selected from the group consisting of esters, alcohols, halides, carboxylic acids, aldehydes, carboxamides, aralkyl, amino and nucleic acids.
6. The compound of Claim 1 wherein R3 and R4 are methyl groups.
7. The compound of Claim 1 wherein R3 and R4 are butyl groups.
8. The compound of Claim 1 wherein the compound is provided in a dosage of between about 25 and about 250 mg compound/kg body weight.
9. The compound of Claim 1 wherein the compound is 2,6-di-tert-butyl-4-(N-tert-octyl) nitronyl phenol.
10. The compound of Claim 1 wherein the compound is 2,6-dimethyl-4-(N-tert-octyl) nitronyl phenol.
11. The compound of Claim 1 wherein the compound is 2,6-di-tert-butyl-4-(N-tert-butyl) nitronyl phenol.
12. The compound of Claim 1 wherein the compound is 2,6-dimethyl-4-(N-tert-butyl) nitronyl phenol.
13. The compound of Claim 1 wherein the compound is N-tert-octyl C-phenyl nitrone.
14. The compound of Claim 1 wherein R1 is hydrogen and R2 is an aryl.
15. The compound of Claim 1 wherein the compound is provided in a dosage of between 25 to 125 mg compound/kg body weight.
16. A compound of a formula:

17. A compound of a formula:

18. A compound having the formula:

wherein R5 is an alkyl having 1 to 4 carbon atoms other than tert-butyl;
R6 is an alkyl having 1 to 4 carbon atoms;
R7 is an alkyl having 1 to 4 carbon atoms;
R8 is an alkyl having 1 to 4 carbon atoms; and R9 is an alkyl having 1 to 4 carbon atoms; for use in the in vivo treatment or prevention of lipid peroxidation.
19. The compound of Claim 18 wherein the compound is provided in a dosage of between 25 mg to 250 mg compound/kg body weight.
20. The compound of Claim 18 wherein the compound is provided in a dosage of between 25 mg to 125 mg compound/kg body weight.
21. The compound of Claim 1 wherein the dosage is from 25 to 50 mg/kg.
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